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基于适配体涂层金纳米粒子和表面酶反应的高灵敏度电化学蛋白质检测。

Highly sensitive electrochemical detection of proteins using aptamer-coated gold nanoparticles and surface enzyme reactions.

机构信息

Department of Chemistry and Green-Nano Materials Research Center, Kyungpook National University, 1370 Sankyuk-dong, Buk-gu, Daegu-city, 702-701, Republic of Korea.

出版信息

Analyst. 2012 May 7;137(9):2011-6. doi: 10.1039/c2an15994e. Epub 2012 Feb 2.

Abstract

A novel electrochemical detection methodology is described for the femtomolar detection of proteins which utilizes both DNA aptamer-functionalized nanoparticles and a surface enzymatic reaction. Immunoglobulin E (IgE) was used as a model protein biomarker, which possesses two distinct epitopes for antibody (anti-IgE) and DNA aptamer binding. A surface sandwich assay format was utilized involving the specific adsorption of IgE onto a gold electrode surface that was pre-modified with a monolayer of aptamer-nanoparticle conjugates followed by the specific interaction of alkaline phosphatase (ALP) conjugated anti-IgE. To clearly demonstrate the signal enhancement associated with nanoparticle use, anodic current measurements of the ALP catalyzed oxidation of the enzyme substrate 4-aminophenylphosphate (APP) were also compared with electrode surfaces upon which the aptamer was directly attached. The detection of an unlabelled protein at concentrations as low as 5 fM is a significant improvement compared to conventional electrochemical-based immunoassay approaches and provides a foundation for the practical use and incorporation of nanoparticle-enhanced detection into electrochemical biosensing technologies.

摘要

一种新颖的电化学检测方法被描述用于检测蛋白质的飞摩尔浓度,该方法利用 DNA 适体功能化纳米粒子和表面酶反应。免疫球蛋白 E(IgE)被用作模型蛋白生物标志物,它具有两个独特的抗体(抗 IgE)和 DNA 适体结合表位。利用表面三明治检测方法,将 IgE 特异性吸附到预先修饰有适体-纳米粒子缀合物单层的金电极表面上,然后特异性地与碱性磷酸酶(ALP)偶联的抗 IgE 相互作用。为了清楚地证明与纳米粒子使用相关的信号增强,还比较了在直接连接适体的电极表面上,ALP 催化酶底物 4-氨基苯磷酸(APP)氧化的阳极电流测量值。与传统基于电化学的免疫分析方法相比,检测未标记蛋白的浓度低至 5 fM 是一个显著的改进,为将纳米粒子增强检测实际应用和纳入电化学生物传感技术奠定了基础。

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